R/events.R
In psichomics: Graphical Interface for Alternative Splicing Quantification, Analysis and Visualisation

Documented in calculateInclusionLevels createJunctionsTemplate getNumerics getSplicingEventCoordinates joinEventsPerType junctionString prepareAnnotationFromEvents prepareGenePresentation sortCoordinates vennEvents

#' @include events_mats.R
#' @include events_miso.R
#' @include events_vastTools.R
#' @include events_suppa.R
NULL

#' Creates a template of alternative splicing junctions
#' 
#' @param nrow Integer: row number
#' @param program Character: program used to get the junctions
#' @param event.type Character: event type
#' @param chromosome Character: chromosome
#' @param strand Character: positive-sense (\code{+}) or negative-sense
#' (\code{-}) strand
#' @param id Character: event identifiers
#' 
#' @return A data frame with the junctions coordinate names pre-filled with
#' \code{NA}
#' @keywords internal
#' 
#' @examples
#' psichomics:::createJunctionsTemplate(nrow = 8)
createJunctionsTemplate <- function(nrow, program = character(0),
                                    event.type = character(0),
                                    chromosome = character(0),
                                    strand = character(0),
                                    id = character(0)) {
    ## TODO(NunoA): only accept a "+" or a "-" strand
    parsed <- as.data.frame(matrix(NA, nrow = nrow, ncol = 8),
                            stringsAsFactors = FALSE)
    names(parsed) <- c("C1.start", "C1.end",
                       "A1.start", "A1.end",
                       "A2.start", "A2.end",
                       "C2.start", "C2.end")
    
    if (length(program) > 0)    parsed[["Program"]] <- "MISO"
    if (length(event.type) > 0) parsed[["Event.type"]] <- event.type
    if (length(chromosome) > 0) parsed[["Chromosome"]] <- chromosome
    if (length(strand) > 0)     parsed[["Strand"]] <- strand
    if (length(id) > 0)         parsed[["Event.ID"]] <- id
    return(parsed)
}

#' Returns the coordinates of interest for a given event type
#' 
#' @param type Character: alternative splicing event type
#' @param sorting Boolean: get coordinates used for sorting and comparison 
#' between different programs?
#' 
#' @return Coordinates of interest according to the alternative splicing event
#' type
#' @keywords internal
getSplicingEventCoordinates <- function(type, sorting=FALSE) {
    coords <- switch(type,
                     "SE"   = c("C1.end", "A1.start", "A1.end", "C2.start"),
                     "A3SS" = c("C1.end", "A2.start", "A1.start"),
                     "A5SS" = c("A2.end", "C2.start", "A1.end"),
                     "AFE"  = c("A2.start", "A2.end", "A1.start", "A1.end"),
                     "ALE"  = c("A1.start", "A1.end", "A2.start", "A2.end"),
                     "RI"   = c("C1.start", "C1.end", "C2.start", "C2.end"),
                     "MXE"  = c("C1.end", "A1.start", "A1.end",
                                "A2.start", "A2.end", "C2.start"),
                     "TandemUTR" = c("A2.start", "A2.end", "A1.end"))
    
    if (sorting) {
        coords <- switch(type,
                         "A3SS" = c("A2.start", "A1.start"),
                         "A5SS" = c("A2.end", "A1.end"),
                         "AFE"  = c("A1.start", "A1.end", "A2.start", "A2.end"),
                         "ALE"  = c("A1.start", "A1.end", "A2.start", "A2.end"),
                         "MXE"  = c("A1.start", "A1.end", "A2.start", "A2.end"),
                         "TandemUTR" = c("A1.end", "A2.end"))
    }
    return(coords)
}

#' Convert a column to numeric if possible and ignore given columns composed
#' of lists
#'
#' @param table Data matrix: table
#' @param by Character: column names of interest
#' @param toNumeric Boolean: which columns to convert to numeric
#'
#' @return Processed data matrix
#' @keywords internal
#' 
#' @examples
#' event <- read.table(text = "ABC123 + 250 300 350
#'                             DEF456 - 900 800 700")
#' names(event) <- c("Event ID", "Strand", "C1.end", "A1.end", "A1.start")
#'
#' # Let's change one column to character
#' event[ , "C1.end"] <- as.character(event[ , "C1.end"])
#' is.character(event[ , "C1.end"])
#'
#' event <- psichomics:::getNumerics(event, by = c("Strand", "C1.end", "A1.end",
#'                                   "A1.start"),
#'                                   toNumeric = c(FALSE, TRUE, TRUE, TRUE))
#' # Let's check if the same column is now integer
#' is.numeric(event[ , "C1.end"])
getNumerics <- function(table, by = NULL, toNumeric = FALSE) {
    # Check which elements are lists of specified length
    bool <- TRUE
    for (each in by)
        bool <- bool & vapply(table[[each]], length, integer(1)) == 1
    
    table <- table[bool, ]
    # Convert elements to numeric
    conv <- by[toNumeric]
    table[conv] <- as.numeric(as.character(unlist(table[conv])))
    return(table)
}

#' Full outer join all given events based on select columns
#' 
#' @param events Data frame or matrix: alternative splicing events
#' @param types Character: alternative splicing types
#' 
#' @importFrom utils txtProgressBar setTxtProgressBar
#' 
#' @return List of events joined by alternative splicing event type
#' @keywords internal
joinEventsPerType <- function(events, types=NULL) {
    if (is.null(types)) types <- names(events)
    
    pb <- txtProgressBar(max=length(types), style=3)
    joinEvents <- function(k, type, events, pb) {
        type <- types[k]
        # Create vector with comparable columns
        id <- c("Strand", "Chromosome", "Event.type")
        by <- c(id, getSplicingEventCoordinates(type))
        toNumeric <- !by %in% id
        
        # Convert given columns to numeric if possible
        tables <- lapply(events[[type]], getNumerics, by, toNumeric)
        
        # Make the names of non-comparable columns distinct
        cols <- lapply(names(tables), function(k) {
            ns <- names(tables[[k]])
            inBy <- ns %in% by
            ifelse(inBy, ns, paste(k, ns, sep="."))
        })
        
        # Full join all the tables
        res <- Reduce(function(x, y) dplyr::full_join(x, y, by), tables)
        names(res) <- unique(unlist(cols))
        
        # Remove equal rows
        res <- unique(res)
        setTxtProgressBar(pb, k)
        return(res)
    }
    joint <- lapply(seq(types), joinEvents, types, events, pb)
    names(joint) <- types
    return(joint)
}

#' Prepare annotation from alternative splicing events
#'
#' In case more than one data frame with alternative splicing events is given,
#' the events are cross-referenced according to the chromosome, strand and 
#' relevant coordinates per event type (see details).
#'
#' @param ... Data frame(s) of alternative splicing events to include in the
#' annotation
#'
#' @details Events from two or more data frames are cross-referenced based on
#' each event's chromosome, strand and specific coordinates relevant for each
#' event type:
#' \itemize{
#'      \item Skipped exon: constitutive exon 1 end, alternative exon (start
#'      and end) and constitutive exon 2 start
#'      \item Mutually exclusive exon: constitutive exon 1 end, alternative exon
#'      1 and 2 (start and end) and constitutive exon 2 start
#'      \item Alternative 5' splice site: constitutive exon 1 end, alternative 
#'      exon 1 end and constitutive exon 2 start
#'      \item Alternative first exon: same as alternative 5' splice site
#'      \item Alternative 3' splice site: constitutive exon 1 end, alternative
#'      exon 1 start and constitutive exon 2 start
#'      \item Alternative last exon: same as alternative 3' splice site
#' }
#'
#' @note When cross-referencing events, gene information is discarded.
#'
#' @importFrom plyr rbind.fill dlply
#'
#' @family functions to prepare alternative splicing annotations
#' @return List of data frames with the annotation from different data frames
#' joined by event type
#' @export
#' 
#' @examples 
#' # Load sample files (SUPPA annotation)
#' folder <- "extdata/eventsAnnotSample/suppa_output/suppaEvents"
#' suppaOutput <- system.file(folder, package="psichomics")
#' 
#' # Parse and prepare SUPPA annotation
#' suppa <- parseSuppaAnnotation(suppaOutput)
#' annot <- prepareAnnotationFromEvents(suppa)
#' 
#' # Load sample files (rMATS annotation)
#' folder <- "extdata/eventsAnnotSample/mats_output/ASEvents/"
#' matsOutput <- system.file(folder, package="psichomics")
#' 
#' # Parse rMATS annotation and prepare combined annotation from rMATS and SUPPA
#' mats <- parseMatsAnnotation(matsOutput)
#' annot <- prepareAnnotationFromEvents(suppa, mats)
prepareAnnotationFromEvents <- function(...) {
    events <- list(...)
    if (!all(vapply(events, is, "ASevents", FUN.VALUE=logical(1))))
        warning("All variables should be an object of class ASevents")
    
    # Remove the "chr" prefix from the chromosome field
    for (each in seq_along(events)) {
        events[[each]]$Chromosome <- gsub("^chr", "", events[[each]]$Chromosome)
    }
    
    # Organise splicing events by event type and then by program in a list of 
    # list of dataframes
    events <- rbind.fill(events)
    events <- dlply(events, "Event.type")
    events <- lapply(events, dlply, "Program")
    
    display("Sorting coordinates...")
    events <- sortCoordinates(events)
    
    display("Joining events per event type...")
    join <- joinEventsPerType(events)
    
    # If available, add 1st constitutive exon's end and 2nd constituve exon's 
    # start from SUPPA or rMATS to AFE and ALE events, respectively, as other 
    # programs may not state these coordinates
    suppaAFE <- join$AFE$SUPPA.C2.start
    matsAFE  <- join$AFE$MATS.C2.start
    AFE.C2.start <- as.numeric( ifelse(
        sapply(suppaAFE, is.null),
        ifelse(sapply(matsAFE, is.null), NA, unlist(matsAFE)),
        unlist(suppaAFE)))
    
    suppaALE <- join$ALE$SUPPA.C1.end
    matsALE  <- join$ALE$MATS.C1.end
    ALE.C1.end <- as.numeric( ifelse(
        sapply(suppaALE, is.null),
        ifelse(sapply(matsALE, is.null), NA, unlist(matsALE)),
        unlist(suppaALE)))
    
    # Organise columns
    organiseCols <- function(i) {
        data <- join[[i]]
        # Include gene column
        geneCol <- grep("Gene$", names(data))
        if (length(geneCol) == 1) {
            gene <- "Gene"
            names(data)[geneCol] <- gene
            data[[gene]] <- as.list(data[[gene]])
        } else if (length(geneCol) == 0) {
            gene <- NULL
        } else {
            gene <- NULL
            # De-prioritise ENSG gene names
            isENSG <- function(col, data) {
                genes <- data[col]
                # Admit that genes are ENSG if over a given threshold
                thershold <- 0.5
                ensg <- grepl("^ENS(G|T)", unique(genes[!is.na(genes)]))
                return(sum(ensg) >= thershold * length(ensg))
            }
            areENSGcols <- sapply(geneCol, isENSG, data)
            geneCol <- c(geneCol[!areENSGcols], geneCol[areENSGcols])
            
            vec <- unlist(data[geneCol])
            names(vec) <- rep(seq(nrow(data)), length(geneCol))
            vec <- vec[!is.na(vec)]
            vec <- vec[unique(names(vec))]
            idx <- as.numeric(names(vec))
            
            gene <- "Gene"
            data[[gene]] <- ""
            data[[gene]][idx] <- vec
        }
        
        cols <- c("Chromosome", "Strand", gene, getSplicingEventCoordinates(i),
                  grep("Event.ID", names(data), value = TRUE))
        return(data[, cols])
    }
    annot <- lapply(names(join), organiseCols)
    names(annot) <- names(join)
    annot$AFE["C2.start"] <- AFE.C2.start
    annot$ALE["C1.end"]   <- ALE.C1.end
    events <- annot
    
    display("Cleaning the annotation...")
    types <- c(SE="Skipped exon", MXE="Mutually exclusive exon",
               A3SS="Alternative 3' splice site", 
               A5SS="Alternative 5' splice site",
               AFE="Alternative first exon", ALE="Alternative last exon",
               RI="Retained intron", TandemUTR="Tandem UTR")
    
    for (type in names(types)) {
        if (!is.null(events[[type]]))
            events[[type]] <- cbind("Event type"=types[[type]], events[[type]])
    }
    events <- rbind.fill(events)
    
    coords <- c("C1.start"="Constitutive exon 1 start",
                "C1.end"="Constitutive exon 1 end",
                "A1.start"="Alternative exon 1 start",
                "A1.end"="Alternative exon 1 end",
                "A2.start"="Alternative exon 2 start",
                "A2.end"="Alternative exon 2 end",
                "C2.start"="Constitutive exon 2 start",
                "C2.end"="Constitutive exon 2 end")
    m <- match(names(coords), names(events))
    names(events)[m[!is.na(m)]] <- coords[!is.na(m)]
    if (is.null(events$Gene)) events$Gene <- NA
    eventId <- grep("Event.ID", names(events), value = TRUE)
    
    # Order rows by event type, chromosome and the first exons coordinates and
    # order columns
    ord <- order(events$`Event type`, events$Chromosome,
                 events$`Constitutive exon 1 start`,
                 events$`Constitutive exon 1 end`,
                 events$`Alternative exon 1 start`,
                 events$`Alternative exon 1 end`)
    events <- events[ord, c("Event type", "Chromosome", "Strand", "Gene",
                            coords[!is.na(m)], eventId)]
    
    # Organise by event type and remove columns with NAs only
    events <- split(events[-1], events$`Event type`)
    for (type in names(events)) {
        naCols <- apply(events[[type]], 2, function(col) all(is.na(col)))
        events[[type]] <- events[[type]][!naCols]
    }
    return(events)
}

#' Compare the number of events from the different programs in a Venn diagram
#' 
#' @param join List of lists of data frame
#' @param eventType Character: type of event
#' 
#' @return Venn diagrams for a given event type
#' @keywords internal
vennEvents <- function(join, eventType) {
    join <- join[[eventType]]
    
    programs <- join[grep("Program", names(join))]
    nas <- !is.na(programs)
    nas <- ifelse(nas, row(nas), NA)
    p <- lapply(seq(ncol(nas)), function(col) nas[!is.na(nas[ , col]), col])
    names(p) <- sapply(programs, function(x) unique(x[!is.na(x)]))
    gplots::venn(p)
}

#' String used to search for matches in a junction quantification file
#'
#' @param chr Character: chromosome
#' @param strand Character: strand
#' @param junc5 Integer: 5' end junction
#' @param junc3 Integer: 3' end junction
#' @param showStrand Boolean: include strand?
#' 
#' @return Formatted character string
#' @keywords internal
junctionString <- function(chr, strand, junc5, junc3, showStrand) {
    plus <- strand == "+"
    first <- ifelse(plus, junc5, junc3)
    last <- ifelse(plus, junc3, junc5)
    if (showStrand)
        res <- sprintf("chr%s:%s:%s:%s", chr, first, last, strand)
    else
        res <- sprintf("chr%s:%s:%s", chr, first, last)
    return(res)
}

colsAsNumbers <- function(type, annotation) {
    # Create vector with comparable columns
    id <- c("Strand", "Chromosome", "Event.type")
    by <- c(id, getSplicingEventCoordinates(type))
    toNumeric <- !by %in% id
    
    # Convert given columns to numeric if possible
    tables <- lapply(annotation[[type]], getNumerics, by, toNumeric)
    return(tables)
}

#' Sort coordinates for some event types
#' 
#' Some programs sort the coordinates of specific event types differently. To
#' make them all comparable across programs, the coordinates are ordered by
#' increasing (plus strand) or decreasing order (minus strand)
#' 
#' @param events List of data frames with alternative splicing events for a 
#' given program
#' 
#' @importFrom utils txtProgressBar setTxtProgressBar
#' 
#' @return List of data frames with alternative splicing events for a given
#' program
#' @keywords internal
sortCoordinates <- function(events) {
    types <- names(events)
    
    progress    <- 0
    maxProgress <- sum(sapply(events, length))
    pb <- txtProgressBar(max=maxProgress, style=3)
    for (type in types) {
        coord          <- getSplicingEventCoordinates(type, sorting=TRUE)
        events[[type]] <- colsAsNumbers(type, events)
        programs       <- names(events[[type]])
        if (!is.null(coord)) {
            for (program in programs) {
                table <- events[[type]][[program]]
                plus  <- table[["Strand"]] == "+"
                plusOrd <- apply(table[plus, coord], 1, sort)
                if (length(plusOrd) > 0) {
                    events[[type]][[program]][plus, coord] <- t(plusOrd)
                }
                minusOrd <- apply(table[!plus, coord], 1, sort, decreasing=TRUE)
                if (length(minusOrd) > 0) {
                    events[[type]][[program]][!plus, coord] <- t(minusOrd)
                }
                progress <- progress + 1
                setTxtProgressBar(pb, progress)
            }
        } else {
            progress <- progress + length(programs)
            setTxtProgressBar(pb, progress)
        }
    }
    return(events)
}

#' Prepare presentation of multiple genes for the same splicing event
#' 
#' @param gene Character: gene
#' @param collapse Character: character string to separate in case of more than
#'   one gene
#' 
#' @return Same object with items collapsed
#' @keywords internal
prepareGenePresentation <- function(gene, collapse="/") {
    multigene <- lapply(gene, length) > 1
    gene[multigene] <- lapply(gene[multigene], paste, collapse=collapse)
    return(gene)
}

prepareEventInfoTooltip <- function(event, data=NULL, pretty=TRUE, ...) {
    parsed <- parseSplicingEvent(event, ..., pretty=pretty, data=data)
    if (is.null(parsed)) return(NULL)
    gene    <- as.character(prepareGenePresentation(parsed$gene,
                                                    collapse=" or "))
    subtype <- parsed$subtype
    strand  <- parsed$strand
    if (!is.null(strand)) {
        strand <- ifelse(strand == "+", "forward", "reverse")
        strand <- sprintf(" (%s strand)", strand)
    } else {
        strand <- ""
    }
    coord <- sprintf("chr %s: %s to %s%s", parsed$chrom,
                     parsed$start, parsed$end, strand)
    res   <- list(gene=gene, subtype=subtype, coord=coord)
    return(res)
}

listPairs <- function(vec1, vec2, vec3=NULL, sorted=FALSE) {
    if (!is.null(vec3)) {
        FUN <- range
    } else if (sorted) {
        FUN <- sort
    } else {
        FUN <- return
    }
    processElems <- function(i, FUN) FUN(c(vec1[[i]], vec2[[i]], vec3[[i]]))
    res <- lapply(seq(length(vec1)), processElems, FUN)
    return(res)
}

#' Calculate inclusion levels using alternative splicing event annotation and
#' junction quantification for many samples
#' 
#' @param eventType Character: type of the alternative event to calculate
#' @param junctionQuant Matrix: junction quantification with samples as columns 
#' and junctions as rows
#' @param annotation Data.frame: alternative splicing annotation related to
#' event type
#' @param minReads Integer: minimum of total reads required to consider the
#' quantification as valid
#' 
#' @importFrom fastmatch fmatch
#' 
#' @return Matrix with inclusion levels
#' @keywords internal
calculateInclusionLevels <- function(eventType, junctionQuant, annotation,
                                     minReads = 10, 
                                     onlyReturnASeventNames = FALSE) {
    # Immediately return NULL if ALE and AFE events are missing coordinates
    if (eventType %in% c("AFE", "AFE_exon") && 
        is.null(annotation$`Constitutive exon 2 start`)) {
        return(NULL)
    } else if (eventType %in% c("ALE", "ALE_exon") && 
               is.null(annotation$`Constitutive exon 1 end`)) {
        return(NULL)
    }
    
    if (is.null(annotation$Gene)) {
        geneCol <- NULL
    } else {
        geneCol <- "Gene"
    }
    gene       <- NULL
    coords     <- rownames(junctionQuant)
    showStrand <- any(grepl("\\+|\\-", coords))
    
    if (eventType == "SE") {
        # Remove duplicates based on columns used to create identifiers
        con1end    <- "Constitutive exon 1 end"
        alt1start  <- "Alternative exon 1 start"
        alt1end    <- "Alternative exon 1 end"
        con2start  <- "Constitutive exon 2 start"
        annotation <- uniqueBy(annotation, "Chromosome", "Strand",
                               con1end, alt1start, alt1end, con2start, geneCol)
        chr    <- annotation$Chromosome
        strand <- annotation$Strand
        if (!is.null(geneCol)) {
            gene <- prepareGenePresentation(annotation[[geneCol]])
        }
        
        con1end    <- annotation[[con1end]]
        alt1start  <- annotation[[alt1start]]
        alt1end    <- annotation[[alt1end]]
        con2start  <- annotation[[con2start]]
        eventNames <- paste(sep="_", eventType, chr, strand, 
                            con1end, alt1start, alt1end, con2start, gene)
        # Prepare event data
        coords_con1 <- I(as.list(con1end))
        coords_alt1 <- I(listPairs(alt1start, alt1end))
        coords_alt2 <- NA
        coords_con2 <- I(as.list(con2start))
        coords_pos  <- I(listPairs(con1end, con2start, sorted=TRUE))
        
        # Create searchable strings for junctions
        incAstr <- junctionString(chr, strand, con1end, alt1start, showStrand)
        incBstr <- junctionString(chr, strand, alt1end, con2start, showStrand)
        excAstr <- junctionString(chr, strand, con1end, con2start, showStrand)
        
        # Get specific junction quantification
        incA <- fmatch(incAstr, coords)
        incB <- fmatch(incBstr, coords)
        excA <- fmatch(excAstr, coords)
        excB <- 0
        
        nas  <- is.na(incA) | is.na(incB) | is.na(excA)
        incA <- incA[!nas]
        incB <- incB[!nas]
        excA <- excA[!nas]
        if (length(incA) == 0) return(NULL)
    } else if (eventType == "MXE") {
        # Remove duplicates based on columns used to create identifiers
        con1end    <- "Constitutive exon 1 end"
        alt1start  <- "Alternative exon 1 start"
        alt1end    <- "Alternative exon 1 end"
        alt2start  <- "Alternative exon 2 start"
        alt2end    <- "Alternative exon 2 end"
        con2start  <- "Constitutive exon 2 start"
        annotation <- uniqueBy(annotation, "Chromosome", "Strand", 
                               con1end, alt1start, alt1end,
                               alt2start, alt2end, con2start, geneCol)
        chr    <- annotation$Chromosome
        strand <- annotation$Strand
        if (!is.null(geneCol)) {
            gene <- prepareGenePresentation(annotation[[geneCol]])
        }
        
        con1end    <- annotation[[con1end]]
        alt1start  <- annotation[[alt1start]]
        alt1end    <- annotation[[alt1end]]
        alt2start  <- annotation[[alt2start]]
        alt2end    <- annotation[[alt2end]]
        con2start  <- annotation[[con2start]]
        eventNames <- paste(sep="_", eventType, chr, strand, 
                            con1end, alt1start, alt1end, 
                            alt2start, alt2end, con2start, gene)
        # Prepare event data
        coords_con1 <- I(as.list(con1end))
        coords_alt1 <- I(listPairs(alt1start, alt1end))
        coords_alt2 <- I(listPairs(alt2start, alt2end))
        coords_con2 <- I(as.list(con2start))
        coords_pos  <- I(listPairs(con1end, con2start, sorted=TRUE))
        
        # Create searchable strings for junctions
        incAstr <- junctionString(chr, strand, con1end, alt1start, showStrand)
        incBstr <- junctionString(chr, strand, alt1end, con2start, showStrand)
        excAstr <- junctionString(chr, strand, con1end, alt2start, showStrand)
        excBstr <- junctionString(chr, strand, alt2end, con2start, showStrand)
        
        # Get specific junction quantification
        incA <- fmatch(incAstr, coords)
        incB <- fmatch(incBstr, coords)
        excA <- fmatch(excAstr, coords)
        excB <- fmatch(excBstr, coords)
        
        nas  <- is.na(incA) | is.na(incB) | is.na(excA) | is.na(excB)
        incA <- incA[!nas]
        incB <- incB[!nas]
        excA <- excA[!nas]
        excB <- excB[!nas]
        if (length(incA) == 0) return(NULL)
    } else if (eventType %in% c("A5SS", "AFE")) {
        alt1end   <- "Alternative exon 1 end"
        alt2end   <- "Alternative exon 2 end"
        con2start <- "Constitutive exon 2 start"
        
        # Backwards compatible with previous annotations
        if (!alt2end %in% names(annotation))
            alt2end <- "Constitutive exon 1 end"
        
        # Remove duplicates based on columns used to create identifiers
        annotation <- annotation[!is.na(annotation[[con2start]]), ]
        annotation <- uniqueBy(annotation, "Chromosome", "Strand",
                               alt2end, alt1end, con2start, geneCol)
        chr    <- annotation$Chromosome
        strand <- annotation$Strand
        if (!is.null(geneCol)) {
            gene <- prepareGenePresentation(annotation[[geneCol]])
        }
        
        alt1end    <- annotation[[alt1end]]
        alt2end    <- annotation[[alt2end]]
        con2start  <- annotation[[con2start]]
        eventNames <- paste(sep="_", eventType, chr, strand, 
                            alt2end, alt1end, con2start, gene)
        # Prepare event data
        coords_con1 <- NA
        coords_alt1 <- I(as.list(alt1end))
        coords_alt2 <- I(as.list(alt2end))
        coords_con2 <- I(as.list(con2start))
        coords_pos  <- I(listPairs(alt1end, alt2end, con2start, sorted=TRUE))
        
        # Create searchable strings for junctions
        incAstr <- junctionString(chr, strand, alt1end, con2start, showStrand)
        excAstr <- junctionString(chr, strand, alt2end, con2start, showStrand)
        
        # Get specific junction quantification
        incA <- fmatch(incAstr, coords)
        incB <- 0
        excA <- fmatch(excAstr, coords)
        excB <- 0
        
        nas  <- is.na(incA) | is.na(excA)
        incA <- incA[!nas]
        excA <- excA[!nas]
        if (length(incA) == 0) return(NULL)
    } else if (eventType %in% c("A3SS", "ALE")) {
        con1end   <- "Constitutive exon 1 end"
        alt1start <- "Alternative exon 1 start"
        alt2start <- "Alternative exon 2 start"
        
        # Backwards compatible with previous annotations
        if (!alt2start %in% names(annotation)) 
            alt2start <- "Constitutive exon 2 start"
        
        # Remove duplicates based on columns used to create identifiers
        annotation <- annotation[!is.na(annotation[[con1end]]), ]
        annotation <- uniqueBy(annotation, "Chromosome", "Strand",
                               con1end, alt1start, alt2start, geneCol)
        chr    <- annotation$Chromosome
        strand <- annotation$Strand
        if (!is.null(geneCol)) {
            gene <- prepareGenePresentation(annotation[[geneCol]])
        }
        
        con1end    <- annotation[[con1end]]
        alt1start  <- annotation[[alt1start]]
        alt2start  <- annotation[[alt2start]]
        eventNames <- paste(sep="_", eventType, chr, strand, 
                            con1end, alt1start, alt2start, gene)
        # Prepare event data
        coords_con1 <- I(as.list(con1end))
        coords_alt1 <- I(as.list(alt1start))
        coords_alt2 <- I(as.list(alt2start))
        coords_con2 <- NA
        coords_pos  <- I(listPairs(con1end, alt1start, alt2start, sorted=TRUE))
        
        # Create searchable strings for junctions
        incAstr <- junctionString(chr, strand, con1end, alt1start, showStrand)
        excAstr <- junctionString(chr, strand, con1end, alt2start, showStrand)
        
        # Get specific junction quantification
        incA <- fmatch(incAstr, coords)
        incB <- 0
        excA <- fmatch(excAstr, coords)
        excB <- 0
        
        nas  <- is.na(incA) | is.na(excA)
        incA <- incA[!nas]
        excA <- excA[!nas]
        if (length(incA) == 0) return(NULL)
    } else if (eventType == "AFE_exon") {
        alt1end      <- "Alternative exon 1 end"
        alt2end      <- "Alternative exon 2 end"
        
        # Backwards compatible with previous annotations
        if (!alt2end %in% names(annotation))
            alt2end <- "Constitutive exon 1 end"
        
        # Remove duplicates based on columns used to create identifiers
        annotation <- uniqueBy(annotation, "Chromosome", "Strand",
                               alt2end, alt1end, geneCol)
        chr    <- annotation$Chromosome
        strand <- annotation$Strand
        if (!is.null(geneCol)) {
            gene <- prepareGenePresentation(annotation[[geneCol]])
        }
        
        alt1end <- annotation[[alt1end]]
        alt2end <- annotation[[alt2end]]
        eventNames <- paste(sep="_", eventType, chr, strand, 
                            alt2end, alt1end, gene)
        # Prepare event data
        coords_con1 <- NA
        coords_alt1 <- I(as.list(alt1end))
        coords_alt2 <- I(as.list(alt2end))
        coords_con2 <- NA
        coords_pos  <- I(listPairs(alt1end, alt2end, sorted=TRUE))
        
        # Create searchable strings for junctions
        incStr <- junctionString(chr, strand, alt1end, "", showStrand)
        excStr <- junctionString(chr, strand, alt2end, "", showStrand)
        coords <- gsub(":[0-9]*:([\\+\\-])$", "::\\1", coords)
        
        # Get specific junction quantification
        inc <- lapply(incStr, grep, coords, fixed=TRUE)
        exc <- lapply(excStr, grep, coords, fixed=TRUE)
        
        nas <- is.na(inc) | is.na(exc)
        inc <- inc[!nas]
        exc <- exc[!nas]
        if (length(inc) == 0) return(NULL)
    } else if (eventType == "ALE_exon") {
        alt1start    <- "Alternative exon 1 start"
        alt2start    <- "Alternative exon 2 start"
        
        # Backwards compatible with previous annotations
        if (!alt2start %in% names(annotation)) 
            alt2start <- "Constitutive exon 2 start"
        
        # Remove duplicates based on columns used to create identifiers
        annotation <- uniqueBy(annotation, "Chromosome", "Strand",
                               alt1start, alt2start, geneCol)
        chr    <- annotation$Chromosome
        strand <- annotation$Strand
        if (!is.null(geneCol)) {
            gene <- prepareGenePresentation(annotation[[geneCol]])
        }
        
        alt1start <- annotation[[alt1start]]
        alt2start <- annotation[[alt2start]]
        eventNames <- paste(sep="_", eventType, chr, strand, 
                            alt1start, alt2start, gene)
        # Prepare event data
        coords_con1 <- NA
        coords_alt1 <- I(as.list(alt1start))
        coords_alt2 <- I(as.list(alt2start))
        coords_con2 <- NA
        coords_pos  <- I(listPairs(alt1start, alt2start, sorted=TRUE))
        
        # Create searchable strings for junctions
        incStr <- junctionString(chr, strand, "", alt1start, showStrand)
        excStr <- junctionString(chr, strand, "", alt2start, showStrand)
        coords <- gsub(":.*?:", "::", coords)
        
        # Get specific junction quantification
        inc <- lapply(incStr, grep, coords, fixed=TRUE)
        exc <- lapply(excStr, grep, coords, fixed=TRUE)
        
        nas <- is.na(inc) | is.na(exc)
        inc <- inc[!nas]
        exc <- exc[!nas]
        if (length(inc) == 0) return(NULL)
    }
    
    if (eventType %in% c("ALE_exon", "AFE_exon")) {
        psi <- psiFastCalc2(junctionQuant, inc=inc, exc=exc, minReads=minReads)
    } else {
        psi <- psiFastCalc(junctionQuant, incA=incA, incB=incB, excA=excA,
                           excB=excB, minReads=minReads)
    }
    
    if (nrow(psi) == 0) return(NULL)
    rownames(psi) <- eventNames[!nas]
    
    # Clear rows with nothing but missing values
    naRows <- rowSums(!is.na(psi)) == 0
    psi    <- psi[!naRows, , drop=FALSE]
    
    # Finalise AS event information
    gene <- NULL
    if (!is.null(geneCol)) gene <- annotation[[geneCol]]
    if (!is.null(gene)) {
        gene <- I(gene)
    } else {
        gene <- NA
    }
    eventData <- data.frame(type=eventType, subtype=eventType, 
                            chrom=chr, strand=strand, gene=gene,
                            start=sapply(coords_pos, min),
                            end=sapply(coords_pos, max),
                            pos=coords_pos,
                            constitutive1=coords_con1,
                            alternative1=coords_alt1,
                            alternative2=coords_alt2,
                            constitutive2=coords_con2)
    rownames(eventData)    <- eventNames
    attr(psi, "eventData") <- eventData[rownames(psi), , drop=FALSE]
    return(psi)
}
Any scripts or data that you put into this service are public.
psichomics documentation built on Nov. 8, 2020, 5:44 p.m.
rdrr.io home R language documentation Run R code online
CRAN packages Bioconductor packages R-Forge packages GitHub packages
Note that we can't provide technical support on individual packages. You should contact the package authors for that.
psichomics
Graphical Interface for Alternative Splicing Quantification, Analysis and Visualisation

R/events.R
In psichomics: Graphical Interface for Alternative Splicing Quantification, Analysis and Visualisation

Defines functions calculateInclusionLevels listPairs prepareEventInfoTooltip prepareGenePresentation sortCoordinates colsAsNumbers junctionString vennEvents prepareAnnotationFromEvents joinEventsPerType getNumerics getSplicingEventCoordinates createJunctionsTemplate

Documented in calculateInclusionLevels createJunctionsTemplate getNumerics getSplicingEventCoordinates joinEventsPerType junctionString prepareAnnotationFromEvents prepareGenePresentation sortCoordinates vennEvents

Try the psichomics package in your browser

R Package Documentation

Browse R Packages

We want your feedback!

psichomics Graphical Interface for Alternative Splicing Quantification, Analysis and Visualisation

R/events.R In psichomics: Graphical Interface for Alternative Splicing Quantification, Analysis and Visualisation

Defines functions calculateInclusionLevels listPairs prepareEventInfoTooltip prepareGenePresentation sortCoordinates colsAsNumbers junctionString vennEvents prepareAnnotationFromEvents joinEventsPerType getNumerics getSplicingEventCoordinates createJunctionsTemplate

Documented in calculateInclusionLevels createJunctionsTemplate getNumerics getSplicingEventCoordinates joinEventsPerType junctionString prepareAnnotationFromEvents prepareGenePresentation sortCoordinates vennEvents

Try the psichomics package in your browser

R Package Documentation

Browse R Packages

We want your feedback!

psichomics
Graphical Interface for Alternative Splicing Quantification, Analysis and Visualisation

R/events.R
In psichomics: Graphical Interface for Alternative Splicing Quantification, Analysis and Visualisation
